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1
Tongue Refolding in the Knotless Cyanobacterial Phytochrome All2699.无结蓝藻植物光敏色素All2699中的舌状重折叠
Biochemistry. 2020 Jun 9;59(22):2047-2054. doi: 10.1021/acs.biochem.0c00209. Epub 2020 Jun 1.
2
MAS NMR on a Red/Far-Red Photochromic Cyanobacteriochrome All2699 from .MAS NMR 研究来自. 的红/远红变色藻胆体 All2699
Int J Mol Sci. 2019 Jul 26;20(15):3656. doi: 10.3390/ijms20153656.
3
Smallest near-infrared fluorescent protein evolved from cyanobacteriochrome as versatile tag for spectral multiplexing.从小型近红外荧光蛋白进化而来的藻胆体作为光谱多重标记的多功能标签。
Nat Commun. 2019 Jan 17;10(1):279. doi: 10.1038/s41467-018-08050-8.
4
The Effective Conjugation Length Is Responsible for the Red/Green Spectral Tuning in the Cyanobacteriochrome Slr1393g3.有效共轭长度决定了蓝藻光色素Slr1393g3中的红/绿光谱调谐。
Angew Chem Int Ed Engl. 2019 Feb 11;58(7):1934-1938. doi: 10.1002/anie.201810266. Epub 2019 Jan 24.
5
Theory and Simulation of the Ultrafast Double-Bond Isomerization of Biological Chromophores.理论与生物发色团超快双键异构化的模拟。
Chem Rev. 2017 Nov 22;117(22):13502-13565. doi: 10.1021/acs.chemrev.7b00177. Epub 2017 Oct 30.
6
The Expanded Red/Green Cyanobacteriochrome Lineage: An Evolutionary Hot Spot.扩展的红/绿藻胆体谱系:进化热点。
Photochem Photobiol. 2017 May;93(3):903-906. doi: 10.1111/php.12764.
7
Phytochrome diversification in cyanobacteria and eukaryotic algae.蓝细菌和真核藻类中的光敏色素多样化。
Curr Opin Plant Biol. 2017 Jun;37:87-93. doi: 10.1016/j.pbi.2017.04.003. Epub 2017 Apr 23.
8
Conformational Homogeneity in the P Isomer of Phytochrome Cph1.植物光敏色素Cph1的P异构体中的构象同质性。
J Phys Chem B. 2017 Mar 30;121(12):2622-2630. doi: 10.1021/acs.jpcb.7b02180. Epub 2017 Mar 16.
9
Bacteriophytochrome Photoisomerization Proceeds Homogeneously Despite Heterogeneity in Ground State.尽管基态存在异质性,但细菌光敏色素的光异构化过程是均匀进行的。
Biophys J. 2016 Nov 15;111(10):2125-2134. doi: 10.1016/j.bpj.2016.10.017.
10
Identification of Cyanobacteriochromes Detecting Far-Red Light.检测远红光的蓝藻光色素的鉴定
Biochemistry. 2016 Jul 19;55(28):3907-19. doi: 10.1021/acs.biochem.6b00299. Epub 2016 Jul 2.

发色团和蛋白质之间的相互作用决定了单结构域光光色素中扩展激发态的动力学。

The interplay between chromophore and protein determines the extended excited state dynamics in a single-domain phytochrome.

机构信息

Institute of Physical and Theoretical Chemistry, Goethe University, D-60438 Frankfurt, Germany;

Institute of Physical and Theoretical Chemistry, Goethe University, D-60438 Frankfurt, Germany.

出版信息

Proc Natl Acad Sci U S A. 2020 Jul 14;117(28):16356-16362. doi: 10.1073/pnas.1921706117. Epub 2020 Jun 26.

DOI:10.1073/pnas.1921706117
PMID:32591422
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC7368379/
Abstract

Phytochromes are a diverse family of bilin-binding photoreceptors that regulate a wide range of physiological processes. Their photochemical properties make them attractive for applications in optogenetics and superresolution microscopy. Phytochromes undergo reversible photoconversion triggered by the ⇄ photoisomerization about the double bond in the bilin chromophore. However, it is not fully understood at the molecular level how the protein framework facilitates the complex photoisomerization dynamics. We have studied a single-domain bilin-binding photoreceptor All2699g1 ( sp. PCC 7120) that exhibits photoconversion between the red light-absorbing (P) and far red-absorbing (P) states just like canonical phytochromes. We present the crystal structure and examine the photoisomerization mechanism of the P form as well as the formation of the primary photoproduct Lumi-R using time-resolved spectroscopy and hybrid quantum mechanics/molecular mechanics simulations. We show that the unusually long excited state lifetime (broad lifetime distribution centered at ∼300 picoseconds) is due to the interactions between the isomerizing pyrrole ring D and an adjacent conserved Tyr142. The decay kinetics shows a strongly distributed character which is imposed by the nonexponential protein dynamics. Our findings offer a mechanistic insight into how the quantum efficiency of the bilin photoisomerization is tuned by the protein environment, thereby providing a structural framework for engineering bilin-based optical agents for imaging and optogenetics applications.

摘要

植物光敏色素是一类多样化的双吡咯环结合光受体,调节着广泛的生理过程。其光化学性质使它们在光遗传学和超分辨率显微镜技术等应用中具有吸引力。植物光敏色素通过双吡咯环发色团中双键的 ⇄ 光异构化触发可逆的光致变色。然而,在分子水平上,蛋白质框架如何促进复杂的光异构化动力学尚不完全清楚。我们研究了一种单结构域双吡咯环结合光受体 All2699g1(sp. PCC 7120),它像典型的植物光敏色素一样在红光吸收(P)和远红光吸收(P)状态之间发生光致变色。我们展示了其晶体结构,并通过时间分辨光谱和混合量子力学/分子力学模拟研究了 P 型的光异构化机制以及初级光产物 Lumi-R 的形成。我们表明,异常长的激发态寿命(约 300 皮秒的宽寿命分布中心)是由于异构吡咯环 D 与相邻保守 Tyr142 之间的相互作用所致。衰减动力学呈现强烈的分布式特征,这是由非指数蛋白动力学强加的。我们的研究结果提供了对双吡咯环光异构化量子效率如何被蛋白质环境调节的机制见解,从而为工程基于双吡咯的光学试剂提供了结构框架,用于成像和光遗传学应用。